Below are detailed procedures for immunohistochemistry and in situ hybridization performed on fresh frozen cryostat cut sections.
Method Article
Immunohistochemistry and in situ hybridization protocols
https://doi.org/10.1038/nprot.2007.510
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Below are detailed procedures for immunohistochemistry and in situ hybridization performed on fresh frozen cryostat cut sections.
Immuno on Cyrostat Sections (Cut sections on Cryostat at 14um)
Day 1: (keep glass tray on ice)
Fix in 4% Para-PBS 10min at 4C for 500 mls: 50 mls 10XPBS, 20g Paraformaldehyde, 11 sodium hydroxide pellets, pH 7.4; filter;)
1XPBS wash at 4C for 5min (repeat wash)
Dry slides especially around where you will write with immedged pen and then place on upside down 96 well plates. Perform the following incubations on the slide itself. Make sure that slides lie flat and solutions do not flow over the Immedged line. Draw a boundary using Immedge pen or place gaskets around sections before starting incubations. Fill tray a little with 1XPBS
Use only BSA when just immunohistochemistry (no Heparin)
Blocking Solution in PBS. Keep BSA in refrigerator.
BSA (Sigma, MB grade) make in 1XPBS 2.5% (0.5g/20mls) 4.8mls
pipette on 250 ul of BSA blocking solution
Cover tray and place in refrigerator. Place slides back into tray.
Rinse in PBS at 4C 3 x 5min
Primary antibody: overnight at 4 C on a level surface in a humid chamber
Antibody solution- in PBS (no Heparin if only immunohistochemistry)
number of slides x 300ul = volume for primary antibody primary Ab:
Triton-X 100 @ 0.1%
BSA @ 1%
Primary antibody 1:1000 dilution (for 5902 VGF Ab)
Day 2 (secondary antibody):
Wash in PBS @ room temperature (RT) 3 X 5 min
secondary antibody incubate for 1 hour at room temperature on a level surface chamber
Solution in 1XPBS
BSA @ 1.0%
Secondary antibody 1:250 dilution (Alexa anti-rabbit)
Wash in 1XPBS 5min
Mounting: wipe off immeged pen around side of slide with a kimwipe, cover slip, and then use Gel/Mount (aqueous mounting medium with anti-fading agents from Biomedia Corp. Cat. # M01)
In Situ Hybridization Protocol
I. T7-PCR based probes for ISH
Making DNA template:
1.Design Forward primer and Reverse primer; reverse primer has a T7 site inserted into the 5’ end. (TAATACGACTCACTATAGG)
2.PCR product approximately 300 bp
3.dilute primers to 10 pmol /ul
4.Use PCR to generate DNA template
II. ISH Protocol
Fixing Protocol:
b. 75% ETOH 2 min
c. 100% ETOH 2 min
Hybridization Buffer for In Situs Day 1
composition: Hyb Buffer (make stock solution and store in freezer);
Making Hybridization Buffer:
100 mls Formamide (American Bioanalytical)
24 mls 5M NaCl (make with DEPC)
2 mls 1M Tris HCl pH 7.4 (make with DEPC)
4 mls 50X Denhardts (from sigma)
5 mls tRNA 10 mg/ml (from sigma)
add 19 mls DEPC water
Mix and pipet out 4 mls into 15 ml falcon tubes (store this stock solution in the freezer)
Preparing Hybridization Buffer:
10% Dextran Sulfate (from a 50% stock solution; so essentially a 80:20 ratio of buffer to dextran sulfate stocks; so for 2ml total volume add 1.6mls hybriization buffer and 0.4mls of dextran sulfate solution)
to this solution add:
Heat probe to 85˚C for 5 minutes before adding to buffer
Example: for up to 15 slides (2 mls total) 1.6 mls HYB buffer stock; 400ul 10% dextran; 20 ul SS DNA; 40ul DTT; **** also once all reagents in hyb buffer leave in 60-70 C oven to ensure that dextran fully dissolves in buffer **** When putting cover slips on tilt at 45 degree angle
Mat Wet Fluid: 10mls 20XSSC; 25mls formamide; make up to 50mls with DEPC H20; use this to keep chambers humid during incubations;
Making Probe (use Mega Shortscript Kit; Ambion Cat # AM1354)
2ul 10X buffer
2ul ATP
2ul GTP
2ul UTP
? ul PCR Product (1ug) heat 3x’s amount to 95 C (5min) to denature PCR product; then add to master mix
2ul T7 polymerase (enzyme)
6 ul 35S CTP
Bring up to 20 ul with DEPC water.
Put into 37 C water bath for 2 hours; Add 1 ul DNAse 1, put back into 37 C water bath for 15 minutes; Then add 45 ul of STE Buffer (STE Buffer: RNase Free; 100mM NaCl; 20mM Tris HCl pH 7.5; 10 mM EDTA; make with DEPC water and store at room temperature) to probe;
Spin columns 1 minute to get rid of buffer (Set centrifuge at 3).
Add probe to spin column. Spin 4 min at 3. Count 1 ul in Scintillation counter.
Second Day In Situ, Washes
b. Wash up and down several times
c. Incubate at room temperature for 30 minutes
RNAse Treatment Buffer Composition
for 200mLs:
0.5 M NaCl 20 mLs 5M NaCl
10mM Tris pH 8.0 2 mLs 1M Tris pH 8.0
1mM EDTA 400 ul 0.5 M EDTA
20ug/ml Rnase 200 uL of 20ug/ul Rnase A
This protocol has been posted on Protocol Exchange, an open repository of community-contributed protocols sponsored by Nature Portfolio. These protocols are posted directly on the Protocol Exchange by authors and are made freely available to the scientific community for use and comment.
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